One concern of phage therapy is the rapid lysing of pathogenic cells which may contain endotoxins. Sudden, masssive releases of toxin can cause dangerous amounts of inflammation. Therefore, phage that kill the targeted pathogen without disrupted the cell's integrity are of interest. This can be accomplished by that by modifying phage to express endonucleases and holins, which are toxic to the cell (chopping DNA and making non-catastrophic disruptions to the cellular membrane)<cite>nonlytic</cite>. Toxin release was minimized, which decreased inflammation and increased the survival rate of treated mice.

One concern of phage therapy is the rapid lysing of pathogenic cells which may contain endotoxins. Sudden, masssive releases of toxin can cause dangerous amounts of inflammation. Therefore, phage that kill the targeted pathogen without disrupted the cell's integrity are of interest. This can be accomplished by that by modifying phage to express endonucleases and holins, which are toxic to the cell (chopping DNA and making non-catastrophic disruptions to the cellular membrane)<cite>nonlytic</cite>. Toxin release was minimized, which decreased inflammation and increased the survival rate of treated mice.

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Phage therapy can also be used in conjunction with antibiotics, even when the target has antibiotic resistance.

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Phage therapy can also be used in conjunction with antibiotics. This is especially useful when trying to avoid quickly evolving resistance to the phage being used. In this approach, the antibiotics provide the killing blow, while the phage assist by suppressing gene networks that are not directly impacted by the antibiotics. One example of this was the combination of ofloxacin (which damage DNA, proteins, and lipids) with phage suppressing the SOS response, which repairs damaged DNA. M13 phage were engineered to overproduce LexA when infecting ''E. coli'', which prevents the SOS response from occurring.

==iGEM==

==iGEM==

Revision as of 01:27, 25 March 2013

Contents

Introduction to Phage Therapy

Phage therapy is the use of viruses to treat bacterial infections. Application of bacteriophage to a bacterial infection will result in the phage infecting, replicating, and then destroying their bacterial hosts. The newly synthesized phage can then go on to infect other bacteria, resulting in the rapid removal of the infection. The use of phages to treat bacterial infections has received new attention due to the appearance of strains of previously treatable pathogens such as methicillin-resistant Staphylococcus aureus, and multidrug-resistant tuberculosis.

History

The discovery of a bacterial-killing substance that could pass through extremely small filters was observed independently several times[1]:

Year

Discoverer, country, microbe sensitive to phage

1896

Hankin, British, Vibrio cholerae

1898

Gamaleya, Russian, Bacillus subtilis

1915

Twort, British, Staphylococcus

1917

d'Herelle, French-Canadian, Shigella

The first therapeutic usage of phage was in 1919, to treat a child with severe dysentery. In a classic case of old-school science, the lead researchers (which included d'Herelle) drank portions of the bacteriophage preparation the day before treating the child, to check the treatment's safety in humans. The researchers didn't keel over, the child fully recovered within a few days, and further tests on other patients confirmed the result.

In the 1930s and 1940s, bacteriophage preparations were developed and sold by major companies such as L'Oréal and the Eli Lilly Company. The development and mass production of antibiotics in the late 1940s halted research into phage therapy in the West, due to the efficacy of antibiotics. Research continued in the Soviet Union. Currently, the only country that has approved phage therapy for human use is Georgia, where the Eliava Institute has researched phage therapy since the 1920s.

Current Applications

Using engineered phage to more efficiently attack a biofilm. The phage carries the gene for DspB, an enzyme that degrades the extracellular polysaccharride component β-1,6-N-acetyl-D-glucosamine. DspB is produced during infection, and released after the cell is lysed, along with new phage.

Regular use of phage therapy occurs primarily in the Republic of Georgia, due to the presence of the Eliava Institute, which has research phage therapy since the 1920s. However, synthetic biology has enabled entirely new approaches to phage therapy, such as engineering new abilities into the phage. One such ability is the degradation of the extracellular polysaccharides (EPS) produced by bacteria during infections[2]. Production of the EPS results in a biofilm, which protects the bacteria within from external harm, such as antibiotics and bacteriophages, limiting the damage to the cells on the surface. To break through this barrier, researches inserted the gene for DspB, an enzyme that degrades one of the key components of EPS. After bacteria on the surface of the biofilm are infected, they produce DspB along with new phage. After the cells lyse, the DspB can degrade the EPS, which exposes more bacteria to infection.

One concern of phage therapy is the rapid lysing of pathogenic cells which may contain endotoxins. Sudden, masssive releases of toxin can cause dangerous amounts of inflammation. Therefore, phage that kill the targeted pathogen without disrupted the cell's integrity are of interest. This can be accomplished by that by modifying phage to express endonucleases and holins, which are toxic to the cell (chopping DNA and making non-catastrophic disruptions to the cellular membrane)[3]. Toxin release was minimized, which decreased inflammation and increased the survival rate of treated mice.

Phage therapy can also be used in conjunction with antibiotics. This is especially useful when trying to avoid quickly evolving resistance to the phage being used. In this approach, the antibiotics provide the killing blow, while the phage assist by suppressing gene networks that are not directly impacted by the antibiotics. One example of this was the combination of ofloxacin (which damage DNA, proteins, and lipids) with phage suppressing the SOS response, which repairs damaged DNA. M13 phage were engineered to overproduce LexA when infecting E. coli, which prevents the SOS response from occurring.

iGEM

Two teams in 2008 had similar approaches to modifying phage therapy: using a host that would be used as a probiotic to carry a phage targeting a gut pathogen. The goal of Team Hiedelberg's "EcoLicense to Kill" was to make a lambda phage that can transfer to a pathogen by conjugation. Once inside the pathogen, the phage would immediately begin replication (due to knocking out the lysogenic cycle of lambda). The pathogen is killed, and phage are released to infect more target bacteria, while leaving the original host (the "killer") unaffected. Team Caltech used a lamB- strain of E. coli that had lambda integrated into it's genome. This was a model for the future application, which could be an E. coli carrying a phage like P22, which could target Salmonella.